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首页> 外文期刊>RNA >Genetic interactions of hypomorphic mutations in the m 7 G cap-binding pocket of yeast nuclear cap binding complex: An essential role for Cbc2 in meiosis via splicing of MER3 pre-mRNA
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Genetic interactions of hypomorphic mutations in the m 7 G cap-binding pocket of yeast nuclear cap binding complex: An essential role for Cbc2 in meiosis via splicing of MER3 pre-mRNA

机译:酵母核帽结合复合体的m 7 G帽结合口袋中的亚型突变的遗传相互作用:通过剪接MER3 pre-mRNA,Cbc2在减数分裂中的重要作用

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摘要

Nuclear cap binding protein complex (CBC) is a heterodimer of a small subunit (Cbc2 in yeast) that binds the m 7G cap and a large subunit (Sto1 in yeast) that interacts with karyopherins. In order to probe the role of cap recognition in yeast CBC function, we introduced alanine mutations (Y24A, F91A, D120A, D122A, R129A, and R133A) and N-terminal deletions (NΔ21 and NΔ42) in the cap-binding pocket of Cbc2. These lesions had no effect on vegetative growth, but they ameliorated the cold-sensitivity of tgs1Δ cells that lack trimethylguanosine caps (a phenotype attributed to ectopic association of CBC with the m 7G cap of the normally TMG-capped U1 snRNA), thereby attesting to their impact on cap binding in vivo. Further studies of the Cbc2-Y24A variant revealed synthetic lethality or sickness with null mutations of proteins involved in early steps of spliceosome assembly (Nam8, Mud1, Swt21, Mud2, Ist3, and Brr1) and with otherwise benign mutations of Msl5, the essential branchpoint binding protein. Whereas the effects of weakening CBC-cap interactions are buffered by other actors in the splicing pathway during mitotic growth, the NΔ42 allele causes a severe impediment to yeast sporulation and meiosis. RNA analysis revealed a selective defect in the splicing of MER3 and SAE3 transcripts in cbc2-NΔ42 diploids during attempted sporulation. An intronless MER3 cDNA fully restored sporulation and spore viability in the cbc2-NΔ42 strain, signifying that MER3 splicing is a limiting transaction. These studies reveal a new level of splicing control during meiosis that is governed by nuclear CBC.
机译:核帽结合蛋白复合物(CBC)是一个小亚基(酵母中的Cbc2)的异二聚体,该亚基结合m 7G帽和一个与核球蛋白相互作用的大亚基(酵母中的Sto1)。为了探讨帽识别在酵母CBC功能中的作用,我们在Cbc2的帽结合口袋中引入了丙氨酸突变(Y24A,F91A,D120A,D122A,R129A和R133A)和N端缺失(NΔ21和NΔ42)。 。这些病变对营养生长没有影响,但是它们改善了缺乏三甲基鸟苷帽(表型归因于CBC与正常TMG封闭的U1 snRNA的m 7G帽异位结合的表型)的tgs1Δ细胞的冷敏性,从而证明了它们对体内帽结合的影响。对Cbc2-Y24A变体的进一步研究显示,合成杀伤力或疾病具有剪接体组装早期步骤中涉及的蛋白质无效突变(Nam8,Mud1,Swt21,Mud2,Ist3和Brr1),而Msl5则是良性突变,是必需的分支点结合蛋白。尽管在有丝分裂生长过程中,剪接途径中其他因子缓冲了CBC-cap相互作用减弱的作用,但NΔ42等位基因严重阻碍了酵母的孢子形成和减数分裂。 RNA分析显示,在尝试形成孢子的过程中,cbc2-NΔ42二倍体中MER3和SAE3转录物的剪接存在选择性缺陷。无内含子的MER3 cDNA完全恢复了cbc2-NΔ42菌株中的孢子形成和孢子活力,这表明MER3剪接是有限的。这些研究揭示了由核CBC控制的减数分裂过程中剪接控制的新水平。

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